This invention covers processes for the isothermal amplification of dna molecules having a preselected sequence. It is based on the unexpected discovery that primers having, at some positions, adenine substituted by 2-aminopurine or diaminopurine, guanine by inosine, thymine by 2-thiothymine, and cytosine by N4-ethylcytosine (“SAMRS nucleotides”) were accepted by enzymes used in the standard helicase-dependent amplification (HDA). Further unexpected was the discovery that target nucleotides are efficiently amplified in an HDA-like process (hereinafter abbreviated as simply HDA) using substituted primers. Also discovered was the diminution of spurious products through the use of SAMRS-substituted primers.
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1. A process for synthesizing a preselected target dna molecule, where said target dna molecule binds to a complementary dna molecule to form a duplex, said process comprising contacting said duplex in buffered aqueous solution with a helicase, a dna polymerase, a single strand binding protein, 2′-deoxynucleoside triphosphates, and a substituted primer, said substituted primer that is complementary in sequence to a segment within said target dna molecule, and where within said substituted primer one adenine in at least one of its 2′-deoxyadenosine nucleotides is substituted by 2-aminopurine or diaminopurine, or one guanine in at least one of its 2′-deoxyguanosine nucleotides is substituted by inosine, or one thymine in at least one of its thymidine nucleotides is substituted by 2-thiothymine, or at least one cytosine in at least one of its 2′-deoxycytidine nucleotides is substituted N4-ethylcytosine, and wherein the total number of said substitutions is between two and six, wherein said polymerase is Bst 2.0, GspSSD, GspM, or GspM2.0.
2. An amplification process for creating multiple copies of a target dna molecule, said process comprising contacting said duplex in buffered aqueous solution with a helicase, a dna polymerase, a single strand binding protein, 2′-deoxynucleoside triphosphates, and two substituted primers, a forward primer and a reverse primer, said forward primer binding to a segment within said target dna molecule, and said reverse primer being substantially identical in sequence to a segment downstream within said target dna molecule, and where within both of said substituted primers one adenine in at least one of its 2′-deoxyadenosine nucleotides is substituted by 2-aminopurine or diaminopurine, or one guanine in at least one of its 2′-deoxyguanosine nucleotides is substituted by inosine, or one thymine in at least one of its thymidine nucleotides is substituted by 2-thiothymine, or at least one cytosine in at least one of its 2′-deoxycytidine nucleotides is substituted by N4-ethylcytosine, and wherein the total number of said substitutions is between two and six, wherein said polymerase is Bst 2.0, GspSSD, GspM, or GspM2.0.
3. The process of
##STR00001##
wherein X is selected from the group consisting of N and CH, W is nitro, cyano, or another electron withdrawing group, and R is the point of attachment of the indicated heterocycle to the oligonucleotide.
4. The process of
##STR00002##
wherein X is selected from the group consisting of N and CH, W is nitro, cyano, or another electron withdrawing group, and R is the point of attachment of the indicated heterocycle to the oligonucleotide.
5. The process of
6. The process of
7. The process of
8. The process of
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This invention was made with government support under a grant awarded by the United States Defense Advanced Research Project Agency (R0011-11-2-0018). The government has certain rights in the invention.
None
Not applicable
None
(1) Field of the Invention
The field of this invention is nucleic acid chemistry, more specifically the field that covers methods for increasing the number of DNA molecules that have a preselected target sequence (“amplifying” that target sequence), and most specifically the field that covers amplification procedures that are done isothermally, without the temperature cycling used in the classical polymerase chain reaction.
(2) Description of Related Art
For practical applications in many areas, including diagnostic procedures that target DNA- and RNA-molecules in biological samples, methods are desired that “amplify” specific nucleic acid sequences. Classically, this has been done by the polymerase chain reaction (PCR) [R. K. Saiki, D. H. Gelfand, S. Stoffel, S. J. Scharf, R. Higuchi, G. T. Horn, K. B. Mullis, H. A. Erlich (1988) Primer-directed enzymatic amplification of DNA with a thermostable DNA polymerase. Science 239, 487-491]. Here, a “forward primer” that binds to a pre-selected target oligonucleotide is annealed to the target sequence to form a duplex. Then, the primer is incubated with a DNA polymerase and the appropriate 2′-deoxynucleoside triphosphates to yield a product that is complementary (in the Watson-Crick sense) to the target oligonucleotides; the target and its complement, as it is formed, are bound in a double stranded double helix. The double strand is then “melted” by heating, typically to temperatures above 75° C., yielding the two complementary DNA strands as single strands. Each strand is freed by heating from its complement. The original target is then able to bind to a second forward primer, while the product DNA molecule is able to bind to a “reverse primer”, which is designed to bind to a preselected site downstream in the product DNA molecule. The polymerase extension is then repeated, with both primers extended to give full-length products, again as duplexes (now two in number). The two strands are then separated by heating to allow more forward and reverse primer to anneal, and the cycle is repeated. The results are multiple copies of both the target DNA molecule and its complement. In asymmetric PCR, the ratio of these two is different from unity.
Classical PCR is widely used throughout research, science, and technology, being the method of choice to detect small amounts of DNA in complex biological samples. Nevertheless, the use of temperature cycling to separate the two strands in product duplexes is undesirable in many applications, including applications that want to amplify target DNA at points-of-care, in doctors offices, and in the field. The desire to amplify target DNA molecules without needing to do repeated temperature cycling is indicated by the literature that searches for amplification methods that do not need temperature cycling, including those known as “recombinase polymerase amplification” (RPA) [Piepenburg, O., Williams, C. H., Stemple, D. L., Armes, N. A. (2006) DNA Detection using recombination proteins. PLoS Biol 4 (7): e204], rolling circle amplification (RCA), NASBA, helicase-dependent amplification (HDA) [Tong, Y., Lemieux, B.,; Kong, H. (2011) Multiple strategies to improve sensitivity, speed and robustness of isothermal nucleic acid amplification for rapid pathogen detection. BMC Biotechnol. 11 Art. No: 50] [Lemieux, B., Li, Y.; Kong, H. M., Tang, Y. W. (2012) Near instrument-free, simple molecular device for rapid detection of herpes simplex viruses: Expert Review Molec. Diagnostics 12, 437-443 DOI: 10.1586/ERM.12.34] and LAMP, among others. These are called “isothermal amplification” methods.
Isothermal amplification methods frequently do not perform well, however. In many cases, the extent of amplification appears to depend on the specific sequence being amplified or (perhaps) the sequence of probes and/or primers used in the amplification. In some cases, the amplification fails entirely. In many cases, extra “spurious” products are observed to arise in addition to the target amplicon. Spurious products are especially seen when isothermal amplification is attempted for more than one target nucleic acid in a single sample (“multiplexing”).
Essentially no theory explains these and other variable results, although speculation can be found in the public and private art, some of it contradictory, other explanations being informal. Without any attempt to be exhaustive, speculative suggestions include the possibility that at low temperatures, non-Watson Crick interactions might cause some of the DNA molecules involved (primer, probe, or analyte) to fold in a way that defeats the amplification process. Others have suggested that high temperatures must be regularly traversed to avoid an (often unknown) intra- or intermolecular interaction from capturing the system as an artifact. Primer-primer interactions have been invoked to explain failure of various isothermal amplification systems, especially when is multiplexing is attempted.
None of these explanations are established. Few data allow us to prefer one over another. As a consequence, the art contains no clear guidance as to what experiments might be tried to overcome these problems, and to generate reliable procedures of performing isothermal amplification for all target sequences and, especially, for multiple (more than one) target sequences.
This is especially true for the isothermal amplification method known as helicase-dependent amplification (HDA). Instead of raising the temperature to separate product duplexes, HDA uses a protein known as helicase. In theory, helicase pulls two strands apart to allow primers to bind to create two duplexes from an original single duplex. While HDA creates successful amplification for many targets, it unfortunately does not for most targets. Again, additional products are often seen with HDA targeting single DNA molecules, often causing the isothermal amplification to fail. Attempts to multiple HDA nearly always fail. Again, while the spurious products are occasionally called “primer dimers”, few if any examples exist where those structures are proven. In any case, formation of these spurious products limits sensitivity and multiplexing. Further, standard HDA cannot use primer concentrations higher than ca. 0.2 μM which limit the speed of detection.
This invention is based on the unexpected discovery that primers (“substituted primers”) in which at least some of the A, T, G, and C nucleobases are substituted at some (but not all) sites (positions) with analogs designated A*, T*, G* and C*, are accepted by enzymes that work together with helicase to effect HDA-like amplification. The presently preferred substitutions replace adenine by 2-aminopurine or diaminopurine (either is defined as A*), replace guanine by inosine (defined as G*), replace thymine by 2-thiothymine (defined as T*), and replace cytosine by N4-ethylcytosine (defined as C*). This invention is further based on the unexpected discovery that target nucleotides are indeed amplified in an HDA-like process (hereinafter abbreviated as simply HDA) using these substituted primers. Further, this invention is based on the discovery that HDA-like processes where its substituted primers are tagged with oligonucleotides incorporating nucleotides selected from as artificially expanded genetic information system (AEGIS, herein defined) also perform well.
1. Narrative
The key inventive feature of this invention are forward and reverse primers where some of their A, T, G, and C nucleobases are substituted at some sites (positions) with analogs designated (respectively) A*, T*, G* and C* (“SAMRS” nucleotides). As is standard in the art, and for both classical and isothermal PCR, the first step in primer design is to select the part, or segment, or sequence of a DNA molecule, for which amplification is sought. The sequence of the forward primers is then selected so that the forward primer is complementary to a part, or segment, of the target sequence, 3′-adjacent to the part of the target that is to be copied. As is also standard in the art, the reverse primer is complementary to a segment “downstream” on the product after the forward primer is extended by template-directed polymerization. As is standard in the art, the forward and reverse primers are designed to give a reasonably sized amplicon product.
References describing the design of sequences of primers to implement classical HDA can be found in the following literature, and references cited therein, which are incorporated in their entirety by citation [Tong, Y., Lemieux, B.,; Kong, H. (2011) Multiple strategies to improve sensitivity, speed and robustness of isothermal nucleic acid amplification for rapid pathogen detection. BMC Biotechnol. 11 Art. No: 50] [Lemieux, B., Li, Y.; Kong, H. M., Tang, Y. W. (2012) Near instrument-free, simple molecular device for rapid detection of herpes simplex viruses: Expert Review Molec. Diagnostics 12, 437-443 DOI: 10.1586/ERM.12.34].
After the primers are chosen to produce the desired amplicon, some of the standard nucleotides in the primer must be substituted by their corresponding SAMRS nucleotide analog. This specification and its examples teach that not all sites should be substituted. Rather, this specification and its examples teach that preferably not fewer than two, and preferably not more than six, substitutions should be made. The presently preferred number of substitutions is four.
Presently preferred are substitutions near the 3′-end of the primer, most preferably at sites n−1, n−2, n−3 . . . , where n is the last, 3′-site in the primer. If the number of SAMRS nucleotides is four, then these are preferably placed at present at sites n−1, n−2, n−3, and n−4, where site n is the 3′-terminal (last) site in the oligonucleotides primer. The presently preferred n substitutions are within the 3′-terminal n+1 sites, the 3′-terminal seven sites for the maximum substitutions (6) and the 3′-terminal three sites for the minimum number of preferred substitutions (2), and the 3′-terminal five sites for most preferred number of substitutions (4).
The presently preferred SAMRS nucleotides replace adenine (A) in the primer by 2-aminopurine or diaminopurine (either is defined as A*), replace guanine (G) in the primer by inosine (defined as G*), replace thymine (T) in the primer by 2-thiothymine (defined as T*), and replace cytosine (C) in the primer by N4-ethylcytosine (defined as C*). Protected phosphoramidites suitable for solid phase DNA synthesis of these nucleoside analogs are well known in the art.
After they are designed, the SAMRS-containing primers are synthesized by solid phase automated synthesis from the corresponding protected phosphoramidites. The methods for synthesizing such primers are described in the following two references, which are incorporated in their entirety herein.
[Hoshika, S., Leal, N., Chen, F., Benner, S. A. (2010) Artificial genetic systems. Self-avoiding DNA in PCR and multiplexed PCR. Angew. Chem. Int. Edit. 49, 5554-5557]
[Yang, Z., Chen, F., Alvarado, J. B., Benner, S. A. (2011) Amplification, mutation, and sequencing of a six-letter synthetic genetic system. J. Am. Chem. Soc. 133, 15105-15112]
Once the primers are prepared, in many of its respects, the isothermal amplification process of the instant invention proceeds just as standard HDA [Tong, Y., Lemieux, B., Kong, H. (2011) Multiple strategies to improve sensitivity, speed and robustness of isothermal nucleic acid amplification for rapid pathogen detection. BMC Biotechnol. 11 Art. No: 50] [Lemieux, B., Li, Y.; Kong, H. M., Tang, Y. W. (2012) Near instrument-free, simple molecular device for rapid detection of herpes simplex viruses: Expert Review Molec. Diagnostics 12, 437-443 DOI: 10.1586/ERM.12.34]. For this reason, the assays are called “HDA-like”. In particular, the invention with its inventive substituted SAMRS primers may be practiced using the helicase enzymes and triphosphates contained in the IsoAmp™ kits sold by BioHelix (Beverly, Mass.) for standard HDA. However, as disclosed in the examples, certain polymerases proved to be exceptionally well suited for the instant invention. Further, optionally, the assay of the instant invention may include single stranded binding protein.
2. Examples
Example 1 describes the amplification of a target DNA molecule (the KIT gene) presented within human genomic DNA (20 ng, corresponding to ca. 6000 copies). This example demonstrated the surprising ability of helicase in conjunction with various polymerases to amplify targets with high efficiency and low noise, even when SAMRS-containing primers were used. It also provided the experimental evidence for the presently preferred use of primers containing four SAMRS nucleotides (G*, C*, T*, and A*), not eight SAMRS nucleotides in the HDA-like process. This example also demonstrated that SAMRS-substituted primers work in this HDA-like assay with different Gsp DNA polymerases (Bst2.0, GspM, Gspm2.0, and GspSSD, all from OptiGene), These experiments further showed that:
The SAMRS-containing primers used in this study are shown below. The bold underlined segments indicate SAMRS substitution, with A* as 2-aminopurine; T* as 2-thio-T; G* as inosine; and C* as N-ethyl-dC.
KIT-90-F-25mer-std:
SEQ ID NO. 1
5′-AGATTTGTGATTTTGGTCTAGCCAG-3′
KIT-90-R-25mer-std:
SEQ ID NO. 2
5′-TGTCAAGCAGAGAATGGGTACTCAC-3′
KIT-90-F-25mer:
SEQ ID NO. 3
5′-AGATTTGTGATTTTGGTCTAGCCAG-3′
KIT-90-R-25mer:
SEQ ID NO. 4
5′-TGTCAAGCAGAGAATGGGTACTCAC-3′
KIT-98-F-29mer:
SEQ ID NO. 5
5′-acaaAGATTTGTGATTTTGGTCTAGCCAG-3′
KIT-98-R-29mer:
SEQ ID NO. 6
5′-ggacTGTCAAGCAGAGAATGGGTACTCAC-3′
These primers were mixed at room temperature with 20 ng of human genomic DNA containing the target DNA sequence as a segment in buffered aqueous solution with a helicase and other components in the IsoAmp mixture from BioHelix (Beverly Mass.), a DNA polymerase from those listed in Table 1, the 2′-deoxynucleoside triphosphates, and various other components listed in Table 1. The mixture was then incubated at 65° C. for 90 min. The conditions are as shown below:
TABLE 1
KIT-
KIT-
SAMRS8-
SAMRS4-
No
KIT Std
25mer
29mer
Template
Final
Components
primers
Primers
Primers
Control
Conc.
dH2O in primer mix
10.5
μL
10.5
μL
10.5
μL
10.5
μL
25
μL
KIT-F-std (5 μM)
1
μL
1
μL
0.2
μM
KIT-R-std (5 μM)
0.2
μM
KIT-F-25mer-SMS (5 μM)
1
μL
1
μL
0.2
μM
KIT-R-25mer-SMS (5 μM)
0.2
μM
KIT-F-29mer-SMS (5 μM)
1
μL
1
μL
0.2
μM
KIT-R-29mer-SMS (5 μM)
0.2
μM
dH2O not in master mix
2
μL
Genomic DNA (10 ng/μL)
2
μL
2
μL
2
μL
20
ng/
25
μL
IsoAmp dNTP Solution
2
μL
2
μL
2
μL
2
μL
1.14×
NaCl (500 mM)
2
μL
2
μL
2
μL
2
μL
40
mM
MgSO4 (100 mM)
1
μL
1
μL
1
μL
1
μL
4
mM
10× Annealing Buffer II
2.5
μL
2.5
μL
2.5
μL
2.5
μL
1×
IsoAmp Enzyme Mix III
2
μL
2
μL
2
μL
2
μL
2×
(BioHelix)
Bst 2.0 (NEB) [8 U/μL]
2
μL
2
μL
2
μL
2
μL
0.64
U/μL
GspM (OptiGene, 8 U/μL)
2
μL
2
μL
2
μL
2
μL
0.64
U/μL
GspM 2.0 (OptiGene, 8 U/μL)
2
μL
2
μL
2
μL
2
μL
0.64
U/μL
GspSSD (OptiGene, 8 U/μL)
2
μL
2
μL
2
μL
2
μL
0.64
U/μL
After each reaction was incubated at 65° C. for 90 min, sample (10 μL) were diluted with a solution loading dye (4 μL). This was loaded as well known in the art on a 2.5% agarose gel. Electrophoresis was used to resolve the PCR products. The results are shown in
The efficiency of a KIT primer pair with four SAMRS bases (G*, C*, T*, and A*) was demonstrated using helicase-dependent amplification (HDA)-like architectures with Bst2.0 and GspSSD and various concentrations of MgSO4 (4 mM, 5 mM, and 6 mM). These experiments showed that:
The primers used in this example are shown below. The underlined bold segments are again the sites where the standard nucleotide was substituted by the corresponding SAMRS nucleotide. Thus, the underlined A indicates A* as DAP (2,6-diaminopurine); the underlined T indicates T* as 2-thio-T; the underlined G indicates G* as inosine; the underlined C indicates C* as N-ethyl-dC.
KIT-98-F-29mer:
SEQ ID NO. 7
5′-acaaAGATTTGTGATTTTGGTCTAGCCAG-3′
KIT-98-R-29mer:
SEQ ID NO. 8
5′-ggacTGTCAAGCAGAGAATGGGTACTCAC-3′
The IsoAmp solution containing polymerases and 2′-deoxynucleoside triphosphates were mixed with the components shown in Table 2 at room temperature. Then, the mixture was incubated at 65° C. for 90 min, sample (10 μL) was diluted with a solution of loading dye (4 μL) and loaded on a 2.5% agarose gel and subjected to electrophoresis to resolve the PCR products. The results are shown in
TABLE 2
KIT-SAMRS-29mer
No Template
Components
Primers
Control
Final Conc.
dH2O in primer mix
10.5
μL
10.5
μL
25
μL
KIT-F-29mer-SMS (5 μM)
1
μL
1
μL
0.2
μM
KIT-R-29mer-SMS (5 μM)
0.2
μM
dH2O not in master mix
2
μL
Genomic DNA (10 ng/μL)
2
μL
0
μL
20
ng/
25
μL
IsoAmp dNTP Solution
2
μL
2
μL
1.14×
NaCl (500 mM)
2
μL
2
μL
40
mM
MgSO4 (100 mM)
1 μL or 1.25 μL or
1 μL or 1.25 μL or
4 mM or 5 mM or
1.5
μL
1.5
μL
6
mM
Betaine (5M)
5
μL
5
μL
1M
10× Annealing Buffer II
2.5
μL
2.5
μL
1×
IsoAmp Enzyme Mix III
2
μL
2
μL
2×
(BioHelix)
Bst 2.0 (NEB) [8 U/μL]
2
μL
2
μL
0.64
U/μL
GspSSD (OptiGene, 8 U/μL)
2
μL
2
μL
0.64
U/μL
This example compared the efficiency and specificity of primers substituted with SAMRS nucleotides (containing G*, C*, T*, and A*) with primers containing only standard nucleotides (no SAMRS nucleotides) to amplify the KIT gene as the target double stranded DNA molecule (presented within whole human Genomic DNA) and HIV DNA (HIV-DNA-96mer, presented as a synthetic simulant) using GspSSD under different concentrations of MgSO4 (6 mM, 7 mM, 8 mM, 9 mM, and 10 mM). In summary, these experiments showed that:
Oligonucleotides used in amplifying KIT gene in human genomic DNA are shown below. The underlined bold A indicates A* as 2-aminopurine; the underlined bold T indicates T* as 2-thio-T; the underlined bold G indicates G* as inosine; the underlined bold C indicates C* as N-ethyl-dC. All components (Table 3, primers, substituted or standard, 2′-deoxynucleoside triphosphates, polymerases, and helicase as part of the IsoAmp kit, obtained from BioHelix), were mixed at room temperature. They were then incubated at 65° C. for 90 min.
KIT-90-F-25mer-std:
SEQ ID NO. 9
5′-AGATTTGTGATTTTGGTCTAGCCAG-3′
KIT-90-R-25mer-std:
SEQ ID NO. 10
5′-TGTCAAGCAGAGAATGGGTACTCAC-3′
KIT-98-F-29mer:
SEQ ID NO. 11
5′-acaaAGATTTGTGATTTTGGTCTAGCCAG-3′
KIT-98-R-29mer:
SEQ ID NO. 12
5′-ggacTGTCAAGCAGAGAATGGGTACTCAC-3′
TABLE 3
No
KIT-Std-
KIT-SAMRS-
Template
Components
Primers
Primers
Control
Final Conc.
dH2O in primer mix
9
μL
9
μL
9
μL
25
μL
KIT-90-F-25mer-Std (5 μM)
1
μL
1
μL
0.2
μM
KIT-90-R-25mer-Std (5 μM)
0.2
μM
KIT-98-F-29mer-SMS (5 μM)
1
μL
1
μL
0.2
μM
KIT-98-R-29mer-SMS (5 μM)
0.2
μM
dH2O in negative control
2
μL
Human Genomic DNA
2
μL
2
μL
20
ng/
(10 ng/μL)
25
μL
IsoAmp dNTP Solution
2
μL
2
μL
2
μL
1.14×
NaCl (500 mM)
2
μL
2
μL
2
μL
40
mM
10× Annealing Buffer II
2.5
μL
2.5
μL
2.5
μL
1×
IsoAmp Enzyme Mix II
2
μL
2
μL
2
μL
2×
(BioHelix)
GspSSD (OptiGene, 8 U/μL)
2
μL
2
μL
2
μL
0.64
U/μL
MgSO4 (100 mM) + H2O
As listed in
As listed in
As listed in
6 mM, 7, 8, 9,
the table
the table
the table
or 10 mM
below
below
below
6 mM
7 mM
8 mM
9 mM
10 mM
MgSO4 (100 mM)
1.5
μL
1.75
μL
2
μL
2.25
μL
2.5
μL
dH2O
1
μL
0.75
μL
0.5
μL
0.25
μL
0
μL
After each reaction was incubated at 65° C. for 90 min, sample (10 μL) was diluted with a solution of plus of loading dye (4 μL), and loaded on a 2.5% agarose gel. Electrophoresis was used to resolve the PCR products. The results are shown in
Oligonucleotides used in amplifying HIV-DNA target are shown below. The underlined bold A indicates A* as 2-aminopurine; the underlined bold T indicates T* as 2-thio-T; the underlined bold G indicates G* as inosine; the underlined bold C indicates C* as N-ethyl-dC. All components (primers, substituted or standard, 2′-deoxynucleoside triphosphates, polymerases, and helicase as part of the IsoAmp kit, obtained from BioHelix), were mixed at room temperature. They were then incubated at 65° C. for 90 min as indicated in Table 4. Primers in this example were extended at their 5′-ends by four nucleotides (indicated by lower case letters):
5′. GagF_Std_30mer:
SEQ ID NO. 13
5′-aaacACCATGCTAAACACAGTGGGGGGACA-3′
6′. GagR_Std_31mer:
SEQ ID NO. 14
5′-atctATCCCATTCTGCAGCTTCCTCATTGAT-3′
5. GagF_SMS_30mer:
SEQ ID NO. 15
5′-aaacACCATGCTAAACACAGTGGGGGGACA-3′
6. GagR_SMS_31mer:
SEQ ID NO. 16
5′-atctATCCCATTCTGCAGCTTCCTCATTGAT-3′
TABLE 4
No
HIV-Std-
HIV-SAMRS-
Template
Components
Primers
Primers
Control
Final Conc.
dH2O in primer mix
9 μL
9 μL
9 μL
25
μL
5′. GagF-Std-30mer (5 μM)
1 μL
1 μL
0.2
μM
6′. GagR-Std-31mer (5 μM)
0.2
μM
5. GagF-SMS-30mer (5 μM)
1 μL
1 μL
0.2
μM
6. GagR-SMS-31mer (5 μM)
0.2
μM
dH2O in negative control
2 μL
HIV-DNA-96mer (0.1
2 μL
2 μL
20
ng/25 μL
fmole/μL)
IsoAmp dNTP Solution
2 μL
2 μL
2 μL
1.14×
NaCl (500 mM)
2 μL
2 μL
2 μL
40
mM
10× Annealing Buffer II
2.5 μL
2.5 μL
2.5 μL
1×
IsoAmp Enzyme Mix II
2 μL
2 μL
2 μL
2×
(BioHelix)
GspSSD (OptiGene, 8 U/μL)
2 μL
2 μL
2 μL
0.64
U/μL
MgSO4 (100 mM) + H2O
As listed in
As listed in the
As listed
6 mM, 7, 8, 9, or
the table
table below
in the
10
mM
below
table
below
Final Mg2+
6 mM
7 mM
8 mM
9 mM
10 mM
(mM)
MgSO4 (100
1.5 μL
1.75 μL
2 μL
2.25 μL
2.5 μL
mM)
dH2O
1 μL
0.75 μL
0.5 μL
0.25 μL
0 μL
After each reaction was incubated at 65° C. for 90 min, sample (10 μL) was diluted with a solution of plus of loading dye (4 μL), and loaded on a 2.5% agarose gel. Electrophoresis was used to resolve the PCR products. The results are shown in
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